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兔肠单个平滑肌细胞中钙储存和瞬时外向电流的特性

Properties of calcium stores and transient outward currents in single smooth muscle cells of rabbit intestine.

作者信息

Bolton T B, Lim S P

机构信息

Department of Pharmacology, St George's Hospital Medical School, London.

出版信息

J Physiol. 1989 Feb;409:385-401. doi: 10.1113/jphysiol.1989.sp017504.

Abstract
  1. Single dispersed cells obtained by collagenase treatment of longitudinal muscle of rabbit small intestine were voltage clamped with low-resistance patch pipettes and membrane current was measured. 2. In cells held at -20 or -30 mV, a discharge of spontaneous transient outward currents (STOCs) was usually seen; these are believed to represent the sporadic release of calcium from storage sites in the cell in relation to TEA-sensitive, 4 AP-resistant, calcium-activated potassium channels. 3. Caffeine (20 mM) externally applied, accelerated and then abolished STOCs; carbachol (0.1 mM) had similar effects; the initial burst of STOCs was often carried on a large, temporary, outward current which could occur alone. This was suggested to be caused by the rapid release of stored calcium in relation to calcium-activated potassium channels. 4. If STOCs were abolished by caffeine (or carbachol) then carbachol (or caffeine) did not evoke outward current indicating that these drugs act on the same calcium store but by different pathways. Inclusion of ryanodine (10(-8)-10(-4) M) in the patch pipette abolished STOCs soon after establishing whole-cell recording mode; afterwards, outward current to caffeine or to carbachol could not be evoked. 5. STOCs were quickly abolished in cells patched with pipettes filled with GTP gamma S (0.1-1 mM) or Gpp(NH)p (0.1-1 mM) but were large or normal in size in cells where GDP beta S (0.1-1 mM) was included in the pipette. GTP gamma S or Gpp(NH)p in the cell abolished outward current to caffeine or to carbachol, but had no effect on calcium-activated potassium channel activity in isolated patches or on a TEA-sensitive, 4-AP-resistant, outward potassium current evoked in single cells by stepping positively from a -20 mV holding potential. These results suggest that the effect of guanine nucleotide analogues are on the calcium store rather than on calcium-activated potassium channels. 6. The effects of GTP gamma S or Gpp(NH)p could be explained if they depleted calcium stores via a G-protein mechanism; this effect may involve activation of phospholipase C enzyme (PLC) and D-myo-inositol 1,4,5-trisphosphate (IP3) production as well as a direct effect on stores. However a separate G-protein-independent pathway of activation of PLC by muscarinic receptor activation may exist as calcium release by carbachol was large or normal in cells filled with GDP beta S.
摘要
  1. 用胶原酶处理兔小肠纵行肌获得的单个分散细胞,用低电阻膜片钳进行电压钳制并测量膜电流。2. 在钳制于-20或-30 mV的细胞中,通常可见自发瞬时外向电流(STOCs)的发放;据信这些电流代表细胞内储存部位钙的散在释放,与TEA敏感、4-AP耐受的钙激活钾通道有关。3. 细胞外施加咖啡因(20 mM),加速然后消除STOCs;卡巴胆碱(0.1 mM)有类似作用;STOCs的初始爆发常伴随着一个大的、暂时的外向电流,该电流可单独出现。提示这是由于储存钙相对于钙激活钾通道的快速释放所致。4. 如果STOCs被咖啡因(或卡巴胆碱)消除,那么卡巴胆碱(或咖啡因)不能诱发外向电流,表明这些药物作用于同一钙储存部位,但通过不同途径。在膜片钳电极中加入ryanodine(10⁻⁸ - 10⁻⁴ M),在建立全细胞记录模式后不久即消除STOCs;此后,不能诱发对咖啡因或卡巴胆碱的外向电流。5. 用充满GTPγS(0.1 - 1 mM)或Gpp(NH)p(0.1 - 1 mM)的电极封接的细胞中,STOCs很快被消除,但在电极中加入GDPβS(0.1 - 1 mM)的细胞中,STOCs大小正常或较大。细胞内的GTPγS或Gpp(NH)p消除了对咖啡因或卡巴胆碱的外向电流,但对分离膜片中的钙激活钾通道活性或从-20 mV钳制电位正向阶跃在单细胞中诱发的TEA敏感、4-AP耐受的外向钾电流无影响。这些结果提示鸟嘌呤核苷酸类似物的作用是在钙储存部位而非钙激活钾通道上。6. 如果GTPγS或Gpp(NH)p通过G蛋白机制耗尽钙储存,其作用就可以得到解释;这种作用可能涉及磷脂酶C(PLC)的激活和D-肌醇-1,4,5-三磷酸(IP₃)的产生以及对储存部位的直接作用。然而,由于在充满GDPβS的细胞中卡巴胆碱引起的钙释放量大或正常,可能存在一条由毒蕈碱受体激活PLC的独立于G蛋白的途径。

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